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Disassembly of actin structures by nanosecond pulsed electric field is a downstream effect of cell swelling

机译:纳秒脉冲电场分解肌动蛋白结构是细胞肿胀的下游效应

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Disruption of the actin cytoskeleton structures was reported as one of the characteristic effects of nanosecondduration pulsed electric field (nsPEF) in both mammalian and plant cells.We utilized CHO cells that expressed the monomeric fluorescent protein (mApple) tagged to actin to test if nsPEF modifies the cell actin directly or as a consequence of cell membrane permeabilization. A train of four 600-ns pulses at 19.2 kV/cm (2 Hz) caused immediate cell membrane poration manifested by YO-PRO-1 dye uptake, gradual cell rounding and swelling. Concurrently, bright actin features were replaced by dimmer and uniform fluorescence of diffuse actin. To block the nsPEF-induced swelling, the bath buffer was isoosmotically supplemented with an electroporeimpermeable solute (sucrose). A similar addition of a smaller, electropore-permeable solute (adonitol) served as a control.We demonstrated that sucrose efficiently blocked disassembly of actin features by nsPEF, whereas adonitol did not. Sucrose also attenuated bleaching of mApple-tagged actin in nsPEF-treated cells (as integrated over the cell volume), although did not fully prevent it. Weconclude that disintegration of the actin cytoskeleton was a result of cell swelling, which, in turn, was caused by cell permeabilization by nsPEF and transmembrane diffusion of solutes which led to the osmotic imbalance.
机译:据报道,肌动蛋白细胞骨架结构的破坏是纳秒持续时间脉冲电场(nsPEF)在哺乳动物和植物细胞中的特征效应之一。我们利用表达标记有肌动蛋白的单体荧光蛋白(mApple)的CHO细胞来测试nsPEF是否修饰细胞肌动蛋白直接作用或细胞膜通透性的结果。一串以19.2 kV / cm(2 Hz)的四个600 ns脉冲引起的立即细胞膜穿孔,表现为YO-PRO-1染料摄取,逐渐的细胞变圆和肿胀。同时,明亮的肌动蛋白特征被弥散性肌动蛋白的调光器和均匀的荧光所取代。为了阻止nsPEF引起的肿胀,在等渗池中补充电渗透不渗透的溶质(蔗糖)。类似地添加了较小的,可通过电孔渗透的溶质(腺苷)作为对照。我们证明了蔗糖有效地阻止了nsPEF阻止肌动蛋白特征的分解,而腺苷醇却没有。蔗糖还减弱了nsPEF处理的细胞中mApple标记的肌动蛋白的漂白(按细胞体积积分),尽管不能完全阻止。我们认为肌动蛋白细胞骨架的崩解是细胞肿胀的结果,而细胞肿胀又是由于nsPEF引起的细胞透化作用和溶质的跨膜扩散引起的,从而导致渗透失衡。

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